Literature DB >> 8527685

Imaging of endosome fusion in BHK fibroblasts based on a novel fluorimetric avidin-biotin binding assay.

N Emans1, J Biwersi, A S Verkman.   

Abstract

A fluorescence assay of in vivo endosome fusion was developed and applied to define the kinetics of endosome fusion in baby hamster kidney (BHK) fibroblasts. The assay is based on an approximately 10-fold enhancement of the green fluorescence of BODIPY-avidin upon biotin binding. The BODIPY-avidin fluorescence enhancement occurred in < 25 ms, was pH-independent, and involved a BODIPY-tryptophan interaction. For endocytosis in vivo, BHK fibroblasts were pulse-labeled with BODIPY-avidin together with a red (rhodamine) fluorescent fusion-independent chromophore (TMR). After specified chase times in a nonfluorescent medium, a second cohort of endosomes was pulse-labeled with biotin-conjugated albumin, dextran, or transferrin. Fusion of biotin-containing endosomes with avidin-containing endosomes was quantified by ratio imaging of BODIPY-to-TMR fluorescence in individual endosomes, using imaging methods developed for endosome pH studies. Analysis of BODIPY-to-TMR ratio distributions in avidin-labeled endosomes exposed to zero and maximum biotin indicated > 90% sensitivity for detection of endosome fusion. In avidin pulse (10 min) -chase-biotin albumin pulse (10 min) studies, both fused and unfused endosomes were identified; the fractions of avidin-labeled endosomes that fused with biotin-labeled endosomes were 0.48, 0.21, 0.16, and 0.07 for 0-, 5-, 10-, and 20-min chase times. Fitting of fusion data to a mathematical model of in vivo endosome fusion required the existence of an intermediate fusion compartment. Pulse-chase studies performed with biotin-transferrin to label the early/recycling endosomes indicated that after a 10-min chase, avidin-labeled endosomes reached a compartment that was inaccessible to biotin-transferrin. The assay was also applied to determine whether endosome fusion was influenced by temperature, pH (bafilomycin A1), second messengers (cAMP agonists, phorbol 12-myristate 13-acetate, staurosporine), and growth-related factors (platelet-derived growth factor, genistein). The results establish a sensitive fluorescence assay to quantify the fusion of vesicular compartments in living cells.

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Year:  1995        PMID: 8527685      PMCID: PMC1236296          DOI: 10.1016/S0006-3495(95)79947-7

Source DB:  PubMed          Journal:  Biophys J        ISSN: 0006-3495            Impact factor:   4.033


  40 in total

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3.  rab5 controls early endosome fusion in vitro.

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Authors:  N A Bradbury; R J Bridges
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Authors:  R J Fallon; M Danaher
Journal:  Exp Cell Res       Date:  1992-12       Impact factor: 3.905

9.  Evidence of a role for heterotrimeric GTP-binding proteins in endosome fusion.

Authors:  M I Colombo; L S Mayorga; P J Casey; P D Stahl
Journal:  Science       Date:  1992-03-27       Impact factor: 47.728

10.  Cell-free fusion of endocytic vesicles is regulated by phosphorylation.

Authors:  P G Woodman; D I Mundy; P Cohen; G Warren
Journal:  J Cell Biol       Date:  1992-01       Impact factor: 10.539

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  14 in total

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4.  Iminobiotin binding induces large fluorescent enhancements in avidin and streptavidin fluorescent conjugates and exhibits diverging pH-dependent binding affinities.

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6.  Cystic fibrosis transmembrane conductance regulator activation stimulates endosome fusion in vivo.

Authors:  J Biwersi; N Emans; A S Verkman
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7.  Multiple lipid compartments slow vesicle contents release in lipases and serum.

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9.  Hybridization of single-stranded DNA targets to immobilized complementary DNA probes: comparison of hairpin versus linear capture probes.

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10.  Heterotypic endosomal fusion as an initial trigger for insulin-induced glucose transporter 4 (GLUT4) translocation in skeletal muscle.

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